>I am having trouble Maxi-prepping pGem4 ( in DH5 ). I'm using the
>Alkaline-lysis method in 'Current-Protocols"
>, repeating Sol,n I,II and III after i have obtained the DNA pellet at the end
>of the crude lysate steps.
>I then do an RNase treatment , 2X P/C/IAA and a P.E.G. precipitation . At ther
>end of all this the plasmid won't
>cut to completion and there is a background smear in the lane of the gel
>,which looks like digested Genomic DNA.
>I know of a few other people who have had trouble with pGem 4 but no sloutions.
If you're willing to go to all that trouble, why not just go one step further
and CsCl band it?
Brett Lindenbach
Program in Immunology
Washington University - St Louis
brett at borcim.wustl.edu